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与RNA结合的hnRNP A1的UP1结构域的首个晶体结构揭示了一种古老RNA结合蛋白的新面貌。

The First Crystal Structure of the UP1 Domain of hnRNP A1 Bound to RNA Reveals a New Look for an Old RNA Binding Protein.

作者信息

Morgan Christopher E, Meagher Jennifer L, Levengood Jeffrey D, Delproposto James, Rollins Carrie, Stuckey Jeanne A, Tolbert Blanton S

机构信息

Department of Chemistry, Case Western Reserve University, Cleveland, OH 44106, USA.

Life Sciences Institute, University of Michigan, Ann Arbor, MI 48109, USA.

出版信息

J Mol Biol. 2015 Oct 9;427(20):3241-3257. doi: 10.1016/j.jmb.2015.05.009. Epub 2015 May 21.

Abstract

The heterogeneous nuclear ribonucleoprotein (hnRNP) A1 protein is a multifunctional RNA binding protein implicated in a wide range of biological functions. Mechanisms and putative hnRNP A1-RNA interactions have been inferred primarily from the crystal structure of its UP1 domain bound to ssDNA. RNA stem loops represent an important class of known hnRNP A1 targets, yet little is known about the structural basis of hnRNP A1-RNA recognition. Here, we report the first high-resolution structure (1.92Å) of UP1 bound to a 5'-AGU-3' trinucleotide that resembles sequence elements of several native hnRNP A1-RNA stem loop targets. UP1 interacts specifically with the AG dinucleotide sequence via a "nucleobase pocket" formed by the β-sheet surface of RRM1 and the inter-RRM linker; RRM2 does not contact the RNA. The inter-RRM linker forms the lid of the nucleobase pocket and we show using structure-guided mutagenesis that the conserved salt-bridge interactions (R75:D155 and R88:D157) on the α-helical side of the RNA binding surface stabilize the linker in a geometry poised to bind RNA. We further investigated the structural basis of UP1 binding HIViSL3(ESS3) by determining a structural model of the complex scored by small-angle X-ray scattering. UP1 docks on the apical loop of SL3(ESS3) using its RRM1 domain and inter-RRM linker only. The biophysical implications of the structural model were tested by measuring kinetic binding parameters, where mutations introduced within the apical loop reduce binding affinities by slowing down the rate of complex formation. Collectively, the data presented here provide the first insights into hnRNP A1-RNA interactions.

摘要

不均一核核糖核蛋白(hnRNP)A1是一种多功能RNA结合蛋白,参与多种生物学功能。hnRNP A1与RNA相互作用的机制主要是根据其与单链DNA结合的UP1结构域的晶体结构推断出来的。RNA茎环是已知的hnRNP A1重要靶标类型,但对于hnRNP A1与RNA识别的结构基础了解甚少。在此,我们报道了UP1与5'-AGU-3'三核苷酸结合的首个高分辨率结构(1.92Å),该三核苷酸类似于几个天然hnRNP A1-RNA茎环靶标的序列元件。UP1通过由RRM1的β-折叠表面和RRM间连接子形成的“核碱基口袋”与AG二核苷酸序列特异性相互作用;RRM2不与RNA接触。RRM间连接子形成核碱基口袋的盖子,我们通过结构导向诱变表明,RNA结合表面α-螺旋侧的保守盐桥相互作用(R75:D155和R88:D157)将连接子稳定在易于结合RNA的几何构象中。我们通过确定经小角X射线散射评分的复合物的结构模型,进一步研究了UP1结合HIViSL3(ESS3)的结构基础。UP1仅使用其RRM1结构域和RRM间连接子停靠在SL3(ESS3)的顶端环上。通过测量动力学结合参数测试了结构模型的生物物理意义,其中在顶端环内引入的突变通过减慢复合物形成速率降低了结合亲和力。总体而言,本文提供的数据首次深入了解了hnRNP A1与RNA的相互作用。

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